From colorless to pink: Structural insights into vitamin B12-induced color change in monoclonal antibodies

单克隆抗体 维生素B12 抗体 单克隆 化学 生物 免疫学 生物化学
作者
Kaifeng He,Haodong Cui,Wenhui Deng,Na Xing,Guo‐Jian Liu,Abdallah Iddy Chaurembo,Li-dan Fu,Yuan Li,Xin-yue Tong,Han-bin Lin,Chunhe Wang
出处
期刊:Medicine in drug discovery [Elsevier BV]
卷期号:28: 100224-100224
标识
DOI:10.1016/j.medidd.2025.100224
摘要

• The pink coloration in monoclonal antibodies (mAbs) arises from light-induced conversion of Vitamin B12 (VB12) to hydroxycobalamin (OH-Cbl), which forms covalent cobalt-sulfur bonds with cysteine residues. • OH-Cbl binds to five cysteine residues: C138 and C218 (light chain), and C22, C96, and C323 (heavy chain), identified via peptide mapping and RP-UPLC/MS. • 3D modeling reveals spacious protein pockets around these cysteines, accommodating VB12′s bulky structure and enabling site-specific covalent attachment. • Hydrophobic interaction chromatography (HIC) and UV absorption (360 nm) confirmed covalent binding, with VB12-supplemented antibodies (SP2) showing higher hydrophobicity and VB12 content (1:5.71 M ratio) than controls (SP1, 1:9.74). • Controlling light exposure during mAb production prevents VB12-to-OH-Cbl conversion, offering a practical solution to avoid coloration and potential quality/safety concerns. Monoclonal antibodies (mAbs) are typically colorless; however, the pink coloration observed during production raises quality concerns. This study investigated the mechanism linking this color change to Vitamin B12 (VB12), which converts to hydroxycobalamin (OH-Cbl) under light and binds covalently to cysteine residues in antibodies via cobalt-sulfur bonds. Two batches of IgG1 antibody (318H3L6)—SP1 (control) and SP2 (VB12-supplemented)—were expressed in CHO cells, exposed to light, and purified. Binding interactions were analyzed using HPLC, RP-UPLC/MS, SDS-PAGE, and hydrophobic interaction chromatography (HIC). Peptide mapping and 3D structural modeling using Modeller software identified the binding sites and spatial requirements. OH-Cbl covalently binds to five cysteine residues: L_Csy138 and L_Csy218 (light chain) and H_Csy22, H_Csy96, and H_Csy323 (heavy chain). SP2 exhibited a higher VB12 content (molar ratio 1:5.71 vs. 1:9.74 in SP1) and increased hydrophobicity, confirming covalent attachment. Structural modeling revealed large protein pockets around these cysteines, accommodating VB12′s bulky structure. Peptide analysis revealed distinct UV absorption at 360 nm for SP2, while SDS-PAGE indicated slight molecular weight differences. The pink coloration arises from the light-induced conversion of VB12 to OH-Cbl, which binds covalently to specific cysteine residues, facilitated by spatially permissive protein pockets. Controlling the light exposure during production can mitigate this phenomenon. This study elucidates the structural basis of antibody-VB12 interactions, offering critical insights for optimizing mAb quality control.
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